IMPLICATIONS OF THE CRYSTALLOGRAPHIC STRUCTURE OF BACTERIORHODOPSIN

Peter Nollert¹, Ehud M. Landau¹, Gabriele Rummel¹, Jurg P. Rosenbusch¹, Eva Pebay-Peyroula²

¹Biozentrum, Basel, Switzerland CH-4056,
²IBS/ESRF, Grenoble, France 38027

Keywords: bacteriorhodopsin; lipidic mesophases; photocycle; proton translocation

An atomic-level understanding of the mechanisms of action of membrane proteins requires the elucidation of their structures to high resolution. To date, only a few high resolution structures of membrane proteins have been solved, reflecting the major obstacle in this endeavor - the routine production of well-ordered three-dimensional crystals. We have developed a novel concept for the crystallization of membrane proteins by exploiting the properties of lipidic mesophases (1).

Bacteriorhodopsin, an integral membrane protein found in the plasma membrane of Halobacterium salinarium was chosen for its advantageous qualities: stability, color, availability and purity. Hexagonal bacteriorhodopsin microcrystals grown in the matrix of a monoolein mesophase diffracted isotropically to 2.0 A resolution, with a space group P6₃, and unit cell dimensions of a=b=61.76 A, c=104.16 A, a=b=90° and g=120°, and one monomer per asymmetric unit. The crystal structure was solved at a resolution of 2.5 A by molecular replacement (2) using previous results from electron crystallographic studies as a model.

The earlier structure is confirmed overall, but several significant differences are revealed. Among those are Arg 82, which in our structure does not seem to form a salt bridge with Asp 85, and Glu 204, whose side chain points away from the putative proton translocation channel. The retinal resides in a hydrophobic pocket, sandwiched between Trp 86 and Trp 182 and is highly bent. Our structure identifies the locations of water molecules and some hydrogen bonds to key residues within this membrane protein in the ground state, which allows to suggest a mechanism of proton translocation in the extracellular side of the protein. In the reprotonation pathway from the cytoplasmic side, distances between key residues are much too large for direct proton transfer and an interpretation will have to await a high resolution structure of a photocycle intermediate.

1. E. M. Landau and J. P. Rosenbusch, Proc. Natl. Acad. Sci. USA, 93, 14532 (1996)
2. E. Pebay-Peyroula, G. Rummel, J. P. Rosenbusch, E. M. Landau, Science 277, 1676 (1997).